Protein-specific glycoform analysis is essential for the thorough understanding of cellular chemistry and signaling but presents a significant assay challenge for small-sized, free-floating exosomes, ubiquitous regulators of cellular physiological functions and mediators of intercellular communication. We report herein a quantitative localized analysis (QLA) method for the first-time achievement of a protein-specific glycosignature assay on these important extracellular vesicles. The integration of localized chemical remodeling and quantitative electrochemistry allows the proof-of-concept QLA examination of exosomal mucin 1 (MUC1)-specific terminal galactose/N-acetylgalactosamine (Gal/GalNAc). In combination with sialic acid (Sia) cleavage manipulation for the exposure of originally capped Gal/GalNAc, QLA has revealed distinct MUC1-specific sialylation capping ratios for MCF-7 and MDA-MB-231 exosomes, as well as when compared to parent cells. These findings suggest a useful noninvasive indicator for subtyping cancer cells and exosome secretion as a likely venue for the preservation of cellular compositional and functional integrity. The QLA method also permits dynamic monitoring of changes in the exosomal MUC1-specific sialylation capping ratio, enabling the distinction of biogenesis pathways of exosomes.Thermal and other transport coefficients were recently shown to be largely independent of the microscopic representation of the energy (current) densities or, more generally, of the relevant conserved densities/currents. In this Article, we show how this gauge invariance, which is intimately related to the intrinsic indeterminacy of the energy of individual atoms in interacting systems, can be exploited to optimize the statistical properties of the current time series from which the transport coefficients are evaluated. To this end, we introduce and exploit a variational principle that relies on the metric properties of the conserved currents, treated as elements of an abstract linear space. Different metrics would result in different variational principles. In particular, we show that a recently proposed data-analysis technique based on the theory of transport in multicomponent systems can be recovered by a suitable choice of this metric.Multireference electron correlation methods describe static and dynamical electron correlation in a balanced way and, therefore, can yield accurate and predictive results even when single-reference methods or multiconfigurational self-consistent field theory fails. One of their most prominent applications in quantum chemistry is the exploration of potential energy surfaces. This includes the optimization of molecular geometries, such as equilibrium geometries and conical intersections and on-the-fly photodynamics simulations, both of which depend heavily on the ability of the method to properly explore the potential energy surface. Because such applications require nuclear gradients and derivative couplings, the availability of analytical nuclear gradients greatly enhances the scope of quantum chemical methods. This review focuses on the developments and advances made in the past two decades. A detailed account of the analytical nuclear gradient and derivative coupling theories is presented. Emphasis is given to the software infrastructure that allows one to make use of these methods. Notable applications of multireference electron correlation methods to chemistry, including geometry optimizations and on-the-fly dynamics, are summarized at the end followed by a discussion of future prospects.A new high-pressure ESI source that can be readily used for commercial API mass spectrometers in a plug-and-play manner without any modification on the ion sampling interface is introduced. The emitter can be operated at ground potential, and the positive mode electrospray is generated by applying a negative high potential to the counter electrode. A shielding electrode effectively shields the opposing electric field and improves the ion transmission. This feature facilitates the direct connection of the ESI emitter to the electrically grounded components. The application of the present ion source to the high-temperature (&gt;100 °C) capillary liquid chromatography for high-speed separation of peptide and proteins is demonstrated using a monolithic polymeric column.A rare example of a dinuclear iron core with a non-linearly bridged dinitrogen ligand is reported in this work. One-electron reduction of [(tBupyrr2py)Fe(OEt2)] (1) (tBupyrr2py2- = 2,6-bis((3,5-di-tert-butyl)pyrrol-2-yl)pyridine) with KC8 yields the complex [K]2[(tBupyrr2py)Fe]2(μ2-η1η1-N2) (2) where the unusual cis-divacant octahedral coordination geometry about each iron and the η5-cation-π coordination of two potassium ions with four pyrrolyl units of the ligand cause distortion of the bridging end-on μ-N2 about the FeN2Fe core. Attempts to generate an Et2O free version of 1 resulted instead in a dinuclear helical dimer [(tBupyrr2py)Fe]2 (3) via bridging of the pyridine moieties of the ligand. Reduction of 3 by two-electrons under N2 does not break up the dimer nor does it result in formation of 2, but instead formation of the ate-complex [K(OEt2)]2[(tBupyrr2py)Fe]2 (4). Reduction of 1 by two-electrons and in the presence of crown-ether forms the tetraanionic N2 complex [K2][K(18-crown-6)]2(tBupyrr2py)Fe]2(μ2-η1η1-N2) (5), also having a distorted FeN2Fe moiety akin to 2. https://www.selleckchem.com/products/jdq443.html Complex 2 is thermally unstable and loses N2, disproportionating to Fe nanoparticles among other products. A combination of single-crystal X-ray diffraction studies, solution and solid state magnetic studies, and 57Fe Mössbauer spectroscopy have been applied to characterize complexes 2-5, whereas DFT studies have been used to help explain the bonding and electronic structure in these unique diiron-N2 complexes 2 and 5.Small, cyclic peptides are reported to have many bioactivities. In bacteria and fungi, they can be made by nonribosomal peptide synthetases, but in plants they are exclusively ribosomal. Cyclic peptides from the Annona genus possess cytotoxic and anti-inflammatory activities, but their biosynthesis is unknown. The medicinal soursop plant, Annona muricata, contains annomuricatins A (cyclo-PGFVSA) and B (cyclo-PNAWLGT). Here, using de novo transcriptomics and tandem mass spectrometry, we identify a suite of short transcripts for precursor proteins for 10 validated annomuricatins, 9 of which are novel. In their precursors, annomuricatins are preceded by an absolutely conserved Glu and each peptide sequence has a conserved proto-C-terminal Pro, revealing parallels with the segetalin orbitides from the seed of Vaccaria hispanica, which are processed through ligation by a prolyl oligopeptidase in a transpeptidation reaction.